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糖皮质激素受体通过阻断NFκB招募P-TEFb来实现启动子特异性转录抑制。

The glucocorticoid receptor blocks P-TEFb recruitment by NFkappaB to effect promoter-specific transcriptional repression.

作者信息

Luecke Hans F, Yamamoto Keith R

机构信息

Department of Cellular and Molecular Pharmacology, University of California-San Francisco, San Francisco, CA 94107-2280, USA.

出版信息

Genes Dev. 2005 May 1;19(9):1116-27. doi: 10.1101/gad.1297105.

DOI:10.1101/gad.1297105
PMID:15879558
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1091745/
Abstract

To investigate the determinants of promoter-specific gene regulation by the glucocorticoid receptor (GR), we compared the composition and function of regulatory complexes at two NFkappaB-responsive genes that are differentially regulated by GR. Transcription of the IL-8 and IkappaBalpha genes is stimulated by TNFalpha in A549 cells, but GR selectively represses IL-8 mRNA synthesis by inhibiting Ser2 phosphorylation of the RNA polymerase II (pol II) C-terminal domain (CTD). The proximal kappaB elements at these genes differ in sequence by a single base pair, and both recruited RelA and p50. Surprisingly, GR was recruited to both of these elements, despite the fact that GR failed to repress the IkappaBalpha promoter. Rather, the regulatory complexes formed at IL-8 and IkappaBalpha were distinguished by differential recruitment of the Ser2 CTD kinase, P-TEFb. Disruption of P-TEFb function by the Cdk-inhibitor, DRB, or by small interfering RNA selectively blocked TNFalpha stimulation of IL-8 mRNA production. GR competed with P-TEFb recruitment to the IL-8 promoter. Strikingly, IL-8 mRNA synthesis was repressed by GR at a post-initiation step, demonstrating that promoter proximal regulatory sequences assemble complexes that impact early and late stages of mRNA synthesis. Thus, GR accomplishes selective repression by targeting promoter-specific components of NFkappaB regulatory complexes.

摘要

为了研究糖皮质激素受体(GR)对启动子特异性基因调控的决定因素,我们比较了GR对两个受NFκB调控且调控方式不同的基因的调控复合物的组成和功能。在A549细胞中,TNFα可刺激IL - 8和IκBα基因的转录,但GR通过抑制RNA聚合酶II(pol II)羧基末端结构域(CTD)的Ser2磷酸化来选择性抑制IL - 8 mRNA的合成。这两个基因的近端κB元件在序列上仅相差一个碱基对,且都能招募RelA和p50。令人惊讶的是,尽管GR未能抑制IκBα启动子,但它仍能被招募到这两个元件上。相反,在IL - 8和IκBα上形成的调控复合物的区别在于Ser2 CTD激酶P - TEFb的募集情况不同。Cdk抑制剂DRB或小干扰RNA破坏P - TEFb的功能可选择性阻断TNFα对IL - 8 mRNA产生的刺激作用。GR与P - TEFb竞争募集到IL - 8启动子上。引人注目的是,GR在起始后步骤抑制IL - 8 mRNA的合成,这表明启动子近端调控序列组装的复合物会影响mRNA合成的早期和晚期阶段。因此,GR通过靶向NFκB调控复合物的启动子特异性成分来实现选择性抑制。

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